不同卵巢运输温度和培养方法对卵母细胞体外成熟的影响

本试验就太谷本地绵羊在卵巢运输温度和培养方法两个方面对绵羊卵母细胞体外成熟的影响作了研究。结果表明，绵羊卵巢在15℃-20℃，22～30℃，32℃-37℃三个运输温度下，以22℃-30℃的A、B级卵母细胞率高，而且卵母细胞的成熟率也最高。培养方法采用传统石蜡油覆盖法和套皿法，发现套皿法的培养效果更好些，可以取代传统的培养方法。     

绵羊卵巢卵母细胞体外成熟培养的研究

在体外受精过程中,绵羊卵巢卵母细胞体外成熟情况在很大程度上决定着卵母细胞的体外受精率和胚胎发育率.影响卵母细胞成熟的因素很多,主要包括卵泡大小、卵巢的发育阶段、培养基、激素生长因子等.试验从屠宰场采集屠宰后的绵羊卵巢,抽取卵巢表面卵泡中的卵母细胞,选择一级和二级卵母细胞进行体外成熟培养.试验证明,绵羊卵巢卵母细胞体外成熟培养时间以24h为佳,FCS浓度以20%最适宜.试验还发现无菌条件、温度、湿度以及在体外对卵母细胞的操作时间对试验的结果都有很大的影响.通过试验初步探明了适宜绵羊卵母细胞体外成熟的一些基本条件,为全面掌握绵羊卵母细胞体外成熟培养以至整个体外受精技术的完善和规范提供了有益的资料.     

发情牛血清对绵羊卵母细胞体外成熟及孤雌胚发育的影响

在动物卵母细胞体外成熟及胚胎体外培养体系中添加一定浓度的发情牛血清可能提高卵母细胞的成熟率及胚胎的发育率。本研究以屠宰场卵巢来源的绵羊卵母细胞为试验材料,探讨了发情牛血清对绵羊卵母细胞体外成熟及孤雌胚发育的影响。结果表明,成熟液中添加10%第1天的发情牛血清能显著提高绵羊卵母细胞的体外成熟率及孤雌胚卵裂率(P＜0.05);孤雌胚体外培养72 h后,向培养液中添加10% 第7天的发情牛血清能显著提高绵羊孤雌胚的桑囊胚率(P＜0.05)。结果表明,发情牛血清能够促进绵羊卵母细胞的体外成熟率及孤雌胚发育率。     

绵羊卵母细胞采集、体外成熟和胚胎体外培养对体外受精技术效率的影响

利用屠宰场采集的绵羊卵巢作为试验材料,研究了不同卵母细胞采集方法(卵泡冲洗法、剖切法、注射器抽吸法和真空泵抽吸法)、成熟液中添加不同来源激素(BIONICHE或宁波激素厂生产 FSH/LH)和血清(发情绵羊血清或胎牛血清),以及mSOF和mCR胚胎培养体系对绵羊体外受精各环节效率的影响。结果表明,卵泡冲洗法获得A、B两级卵母细胞比例为77.1%,显著高于其他3种方法(P＜0.05),添加BIONICHE FSH/LH+ESS成熟液中,卵母细胞成熟率显著高于其他添加方式(P＜0.05),mSOF和mCR胚胎培养体系在卵裂率上无显著差异(P＞0.05),但mSOF组中囊胚率和孵化率均显著高于mCR组(P＜0.05)。综上所述,本研究中卵泡冲洗法更适合绵羊卵母细胞采集,成熟液中添加BIONICHE FSH/LH和ESS可显著促进绵羊卵母细胞成熟;与mCR培养体系相比,mSOF培养体系更适合绵羊体外受精胚胎的发育。     

铁对牛卵母细胞体外成熟和体外受精的影响

本试验研究铁对体外生产牛胚胎的影响。从屠宰场收集牛卵巢,抽取卵巢表面的卵母细胞,采用体外成熟和体外受精的方法,研究不同浓度的铁(0.45mg/L,0.81mg/L,1.96mg/L,2.78mg/L)对牛卵母细胞体外成熟和体外受精的影响。结果如下:当卵母细胞在体外培养22h时,不同浓度的铁之间对卵母细胞体外成熟影响较小,差异不显著(p>0.05),且与对照组之间差异不显著(p>0.05);在体外受精的研究中,铁浓度为1.96mg/L和2.78mg/L的受精卵培养液可以明显提高8细胞胚胎发育率,差异显著(p<0.05);铁浓度为1.96mg/L的受精卵培养液可以明显提高囊胚发育率,囊胚发育率为31.6%,与其他浓度的铁相比,差异显著(p<0.05)。本试验结果说明:在卵母细胞体外成熟阶段,培养液中的铁对卵母细胞体外成熟没有影响,但对受精后早期胚胎的发育有促进作用,1.96mg/L是比较合适的早期胚胎培养液中铁的添加量。     

血管内皮生长因子对绵羊卵母细胞体外成熟及体外受精卵卵裂率的影响

试验研究了在绵羊体外成熟和体外受精培养系统中分别添加5ng/mL血管内皮生长因子(VEGF)对绵羊卵母细胞体外成熟和体外受精卵的早期发育的影响。结果表明:①与对照组相比,添加5ng/mLVEGF能够显著(P<0.01)提高绵羊卵母细胞的体外成熟率。②在体外受精液中添加5ng/mLVEGF能够显著(P<0.05)提高成熟卵母细胞的卵裂率。研究表明,VEGF对绵羊卵母细胞的体外成熟和受精具有调节作用。     

维生素C对獭兔卵母细胞体外成熟的影响

目的：为了探讨Vc浓度对獭兔的卵母细胞体外成熟的影响,本实验采用不同浓度Vc处理獭兔卵母细胞,观察细胞体外成熟培养成熟率。方法：去獭兔场取现屠宰的獭兔的卵巢后,用机械切割法得到卵母细胞,然后把获取的细胞放入加了3个不同Vc浓度的M199培养基进行培养,低浓度（0.25mg/ml）、中浓度（0.5mg/ml）、高浓度（0.75mg/ml）,培养液在温度37℃、湿度100%、CO2浓度5%的CO2培养箱中进行培养;结果：卵母细胞成熟率,低浓度、中浓度、高浓度、对照组分别为41.67%、47.61%、33.33%、46.67%,4组之间差异均不显著（P〉0.05）;结论：不同浓度Vc对獭兔的卵母细胞体外成熟培养无明显影响,但中浓度Vc卵母细胞成熟率最低。     

猪卵巢卵母细胞的体外成熟和体外受精

将从屠宰母猪卵巢采得的卵母细胞-卵丘细胞复合体(Oocyte-cumulus Cell Complex.OCC)在含PMSG的M199培养40～44小时,卵丘细胞大部分扩散(86.4％)。48.1％(142/295)的卵母细胞排出第一极体(PBI)。将体外成熟的卵母细胞与体外获能精子授精后30～70小时,80.5％(103/128)的卵母细胞受精并可在体外发育到2～8细胞甚至桑椹胚。本文还对裸卵母细胞的体外成熟和体外受精进行了研究,对体外受精卵的早期发育作了观察。实验结果表明:PMSG对诱导卵丘细胞扩散及卵母细胞的全面成熟有重要作用,在OCC中的卵母细胞成熟率高于裸卵母细胞体外授精后8～10小时将受精卵放入改良KRB液培养可使卵裂比例明显提高。     

细胞松弛素B对绵羊GV期卵母细胞玻璃化冷冻效果的影响

本试验通过玻璃化冷冻前细胞松弛素B(CB)预处理来分析CB对绵羊GV期卵母细胞玻璃化冷冻/解冻后发育潜力的影响。分别从细胞毒性检测、冷冻检测和CB不同浓度（6.0、7.5和9.0 μg/ml）处理3个方面进行试验。试验结果表明毒性检验中CB处理组和未处理组卵母细胞的成熟率都显著低于对照组(P<0.05)，但相互之间差异不显著；玻璃化冷冻后，卵母细胞成熟率显著低于未冷冻组(P<0.05)，玻璃化冷冻CB处理组和未处理组卵母细胞体外成熟培养后成熟率之间差异不显著(P>0.05)；不同CB浓度处理后9.0 μg/ml组卵母细胞的成熟率显著高于对照组（P<0.05）。     

马尾藻属藻类多糖对猪卵母细胞体外成熟及凋亡的影响

本研究就马尾藻属藻类多糖对猪卵母细胞的体外成熟及凋亡进行了探索：试验一证明，体外培养46h～48h时，成熟液添加马尾藻属藻类多糖能促进卵丘细胞扩展，添加20mg/ml马尾藻属藻类多糖能提高核成熟率(41．8%)，与对照组29．3%的核成熟率相比，二者差异显著；试验二证明，添加马尾藻属藻类多糖可延长猪卵母细胞体外存活时问，体外培养第16d，在含有0、5mg/ml、20mg/ml马尾藻属藻类多糖培养液中的猪卵母细胞存活率分别为2．6%、18．9%、23．0%，添加与否差异显著。     

血清和促性腺激素对山羊卵母细胞核体外成熟的影响

试验研究了清和促性腺激素对山羊卵丘扩展和卵母细胞核成熟的,卵母细胞与卵丘扩展的关系以及卵丘扩展与卵母细胞核成熟的关系。结果表明：（1）培养24h，添加PMSG组卵母细胞核成熟率显著高于不加激素组（P＜0．05），而培养到27h，2者成熟率之间差异变得不显著，说明添加PMSG卵母细胞核的最终成熟率没有明显影响，但加速了卵母细胞核的成熟进程；（2）M199＋BSA培养27h，卵母细胞核成熟率显著高于培养24h，而M199＋FCS培养27h与培养24h的成熟差异不显著，说明添加BSA时，卵母细胞核体外成熟速度比添加FCS的慢；（3）卵丘扩展良好与扩展不好的卵母细胞核成熟率以及第1极体形态无统计学差异，说明山羊卵母细胞的核成熟可能不依赖于卵丘扩展；（4）山羊的卵丘扩展产不依赖于卵母细胞；（5）将带壁颗粒细胞与不带壁颗粒细胞的COC分开培养发现，2者卵母细胞核成熟度无明显差异，带有壁颗粒细胞的COC卵丘扩展情况明显优于一般COC。     

海狸鼠卵母细胞体外成熟培养初探

实验用ＰＭＳＧ或ＰＭＳＧ＋ＨＣＧ处理或未经激素处理的海狸鼠８只，共获卵巢卵母细胞１３８枚。激素处理对获取卵巢卵母细胞的数量没有影响，而对体外成熟发育至卵丘扩展和半成熟阶段有促进作用。三种不同培养液（Ｗｈｉｔｅｎ＋ＦＣＳ；ＴＣＭ１９９＋ＰＭＳＧ＋ＦＣＳ；ＴＣＭ１９９＋ＨＣＧ＋ＦＣＳ）共培养１２５枚卵母细胞，培养后卵丘扩展率及半成熟率分别为５６．５％，４５．７％，４７．６％和２１．７％，１２．３％，９．５％，以Ｗｈｉｔｅｎ液较高（分别为５６．５％和２１．７％），但只有ＴＣＭ１９９＋ＰＭＳＧ＋ＦＣＳ组有２枚卵母细胞出现第一极体。结果表明海狸鼠卵母细胞与其它啮齿动物的卵母细胞一样，能够在体外培养成熟，完成第一次减数分裂，排出第一极体     

Time Course of In Vitro Maturation of Compact Cumulus Horse Oocytes after Roscovitine‐Induced Meiotic Inhibition: Effects on the Coordination Between Nuclear and Cytoplasmic Maturation

This study was carried out to evaluate the usefulness of a pre‐maturation step in improving the coordination between cytoplasmic and nuclear maturation of horse compact cumulus oocytes by the addition of roscovitine (ROSC). Oocytes were collected by scraping and pre‐cultured for 18 h in a maturation medium TCM199 supplemented with pyruvate, LH, FSH, insulin growth factor (IGF), epidermal growth factor (EGF), insulin, transferrin and selenium (IVM‐ROSC) or in a simple medium (M199‐ROSC). After pre‐maturation, oocytes from both the groups were in part denuded and fixed‐stained and in part in vitro matured to assess the kinetic of in vitro maturation (IVM). The nuclear progression and the cytoskeletal organization of microfilaments and cortical granules (CG) of treated and untreated oocytes were assessed by fluorescent probes. Oocytes immediately fixed after recovery and oocytes pre‐cultured in M199‐ROSC for 18 h did not show metaphase II (MII) plates, whereas in IVM‐ROSC group, 6/69 oocytes (8.7%) showed MII plates. After inhibition, during maturation kinetics at 11, 18 and 29 h, maturation rate of M199‐ROSC group progressively increased and at 29 h of IVM, reached the maturation rate of control group (13/66, 19.7% vs 31/125, 24.8%). No statistically significant differences in cytoplasmic maturation were found. The number of MII plates after 29 h of IVM, was significantly higher (p < 0.05) in IVM‐ROSC group (34/90) compared with M199‐ROSC (13/66) and control groups (31/125) as well as the number of oocytes with microfilaments and CG distributed in cortical region (25/34 vs 3/13 and 7/31 respectively). Our results showed that pre‐culturing in the presence of Roscovitine in a fully supplemented maturation medium containing gonadotropins and growth factors partially suppressed the meiotic maturation, but established a more suitable environment for improving cytoplasmic maturation of horse compact cumulus oocytes as defined by microfilaments and CG configuration.     

绵羊卵泡卵体外成熟的研究

本研究主要探讨了不同激素、卵母细胞形态及入培前时间对绵羊卵泡卵体外成熟效果的影响.结果表明:卵母细胞在添加FSH LH(均为10IU/mL)、HCG(4IU/mL)及不加激素的m—TCM199 10％FCS(V/V)培养液中培养24h后,达到中期Ⅱ的卵母细胞比例分别为87.68％、96.00％和42.11％;卵母细胞的形态是影响其成熟的重要因素,A、B、C三级卵培养24h后的成熟率分别为91.77％、57.10％和25.84％,入培前时间间隔为2、4、8h时,其成熟率分别为80.24％、77.42％和 77.83％,相互间差异不显著(P>0.05).     

培养介质、卵丘细胞和卵泡直径对猪卵母细胞体外成熟的影响

A类卵母细胞在mTCM 199、NCSU2 3和NCSU37体系中培养 4 4～ 5 2小时后 ,成熟率分别为 76 .1%、78.1%和 6 5 .2 %。前两者差异不显著 (P >0 .0 5 ) ,但显著高于后者 (P <0 .0 5 )。卵母细胞在添加eCG和hCG的NCSU2 3体系中的成熟率 (75 .6 % )明显高于添加FSH的LH和成熟率 (6 5 .2 % ) (P <0 .0 5 )。A、B、C三类卵母细胞在NCSU2 3的成熟率分别为 73.3%、6 0 .4 %和 11.0 % ,三者间差异显著 (P <0 .0 5 )。大 (ф >6mm)、中 (ф =3～ 6mm)和小 (ф <3mm)三种卵泡中的卵母细胞在NCSU2 3中培养后 ,成熟率分别为 5 6 .2 % ,78.1%和 5 1.9% ,中等卵泡中卵母胞的体外成熟率显著高于其他两组 (P <0 .0 5 )。     

Influence of follicle size,methods of retrieval on oocytes yield and morphology in Egyptian Jennies ovaries with special reference to maturation rate in vitro

This work was designed to evaluate the ovarian follicular development, oocytes morphology, methods of oocytes reterival, and the effect of different in vitro maturation (IVM) media on cumulus cell expansion and nuclear maturation of Jennies oocytes. Experiment 1, the number of small (<6 mm), medium (6 to 9 mm) and large size (>10 mm) ovarian follicles was recorded. Cumulus-oocyte-complexes (COCs) were reterived and classified into 4 Grades based on their cumulus-cells investment and the homogenous of the ooplasm. In Experiment 2, COCs were recovered by using 18-G, 20-G needle or slicing and scraping of ovarian follicles to determine the number and morphology of the recovered COCs. In Experiment 3, Grade A and B COCs were IVM in DMEM-HG, DMEM-LG, DMEM-F12, TCM199, TCM199-F12 or CR1aa media supplemented with 10 % FCS?+?10 μg FSH/mL?+?10 IU hCG/mL?+?50 μg/mL gentamicin. Maturation was performed for 36 h at 38.5 °C under 5 % CO₂ in humidified air. After IVM, cumulus cell expansion and oocytes nuclear canfiguration were determined. An average of 6.40?±?0.26 follicles was recorded per Jenny ovary, representing 3.37?±?0.46, 1.89?±?0.14 and 1.14?±?0.16, for the small, medium and large size follicles, respectively. Oocyte recovery was higher (P?P?P?P?P?P?P?P?Conclusion: Slicing and scraping or aspiration of follicles using 18-G needle increased the number and percentage of Grade A Jennies oocytes. TCM199-F12, CR1aa and TCM199 medi are more suitable for IVM of Jenny oocytes by promoting cumulus cells expansion and nuclear maturation to M II stage.     

Elevated Histone H1 (MPF) and Mitogen-activated Protein Kinase Activities in Pig Oocytes Following In Vitro Maturation do not Indicate Cytoplasmic Maturation

Effects of different media (TCM 199 + BSA, TCM 199 + FCS, TCM 199 + NBCS, Whitten's medium + BSA) supplemented with estradiol-17β and two isolated and everted follicle shells on MPF and MAP kinase activities and the sensitivity to parthenogenetic activation of pig oocytes were examined at the end of culture (48 h). Elevated ( P  <   0.05) activities of MAP kinase were recorded in metaphase II oocytes following culture in Whitten's medium, whereas MPF levels were lowest ( P  <   0.05) in MII oocytes matured in TCM 199 supplemented with BSA. Oocytes matured in TCM 199 based media showed higher ( P  <   0.05) activation rates when compared to oocytes incubated in Whitten's medium. Whitten's medium supplemented with different protein sources (amino acids, FCS, BSA) was used to study the effects of different exposure periods to eCG/hCG stimulation on MPF and MAP kinase activities and in vivo fertilisability following culture for 48 h. MPF and MAP kinase activities were significantly increased by eCG/hCG stimulation of COCs during maturation. Further, the continuous presence of eCG/hCG during culture (48 h) significantly increased the levels of both kinases in comparison to stimulation by gonadotrophins alone during the first 24 h of incubation. In vivo fertilisation of oocytes matured in Whitten's medium supplemented with eCG/hCG for 24 or 48 h led to a significant retardation of early embryonic development compared to ovulated oocytes. In conclusion, media composition and gonadotrophin stimulation affect MPF/MAP kinase activities and the susceptibility to parthenogenetic activation of IVM oocytes. However, elevated kinase levels in pig oocytes following culture do not indicate complete cytoplasmic maturation.     

Attempt at in vitro maturation of minke whale (Balaenoptera Bonaerensis) oocytes using a portable CO2 incubator

The present study was conducted to investigate whether a portable CO2 incubator was effective for in vitro maturation (IVM) of bovine, porcine and minke whale oocytes, and the effect of maturation media supplemented with different hormones; porcine follicle stimulating hormone (pFSH), estradiol-17beta (E2), or pregnant mare's serum gonadotropin (PMSG): human chorionic gonadotropin (hCG) for minke whale immature oocytes was also examined. In vitro maturation rates of bovine and porcine oocytes cultured in the portable CO2 incubator were not significantly different from the standard CO2 incubator. In minke whale IVM culture using the portable incubator, the maximum expansion of cumulus mass was observed by pFSH/E2 and PMSG/hCG at the end of IVM culture. Moreover, the IVM culture period was shortened to 28-30 h from 96-120 h previously reported. The proportion of matured oocytes cultured in the medium supplemented with pFSH/E2 (26.7%) was significantly higher (P<0.05) than that with PMSG/hCG (6.9%). The present study indicates that a portable CO2 incubator is a useful device for minke whale IVM culture on a research base ship, and the addition of pFSH/E2 into an IVM medium enhanced cumulus expansion and the proportion of minke whale matured oocytes.     

Cumulus Expansion, in vitro Fertilization and Embryonic Development after in vitro Maturation of Bovine Oocytes in the Presence of Follicle Stimulating or Luteinizing Hormone

Contents: Bovine follicular oocytes were matured and fertilize din vitro. The frequency of penetration and subsequent embryonic development were improved considerably, for oocytes cultured in larger volumes allowing larger oocyte groups as compared to the culture of 2 oocytes within 30 μl drops. The effects of follicle stimulating hormone (FSH) and luteinizing hormone (LH), present during in vitro maturation, were studied in terms of cumulus expansion, oocyte penetration, male pronucleus formation and embryonic development. Cumulus expansion including mucification was induced by both hormones. Scanning electron microgfaphs revealed that storage of LH as a frozen solution over a long time period (10 months), destroyed its ability to stimulate cumulus mucification, whereas uncoupling of the cumulus cell processes still occurred. LH caused an increase in the percentage of penetrated oocytes with incomplete sperm head decondensation. This effect was also lost after long term storage. Teh resulting total penetration frequency as well as the proportion of oocytes with both pronuclei formed was now similar to that observed with oocytes matured with fresh LH or FSH. Embryonic development was not altered by the replacement of FSH by LH during in vitro maturation .